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Rab5活性成像确定了吞噬体成熟的关键调节因子。

Imaging of Rab5 activity identifies essential regulators for phagosome maturation.

作者信息

Kitano Masahiro, Nakaya Michio, Nakamura Takeshi, Nagata Shigekazu, Matsuda Michiyuki

机构信息

Laboratory of Bioimaging and Cell Signaling, Graduate School of Biostudies, Kyoto University, Yoshida Konoe-cho, Sakyo-ku, Kyoto 606-8501, Japan.

出版信息

Nature. 2008 May 8;453(7192):241-5. doi: 10.1038/nature06857. Epub 2008 Apr 2.

DOI:10.1038/nature06857
PMID:18385674
Abstract

Efficient phagocytosis of apoptotic cells is crucial for tissue homeostasis and the immune response. Rab5 is known as a key regulator of the early endocytic pathway and we have recently shown that Rab5 is also implicated in apoptotic cell engulfment; however, the precise spatio-temporal dynamics of Rab5 activity remain unknown. Here, using a newly developed fluorescence resonance energy transfer biosensor, we describe a change in Rab5 activity during the engulfment of apoptotic thymocytes. Rab5 activity on phagosome membranes began to increase on disassembly of the actin coat encapsulating phagosomes. Rab5 activation was either continuous or repetitive for up to 10 min, but it ended before the collapse of engulfed apoptotic cells. Expression of a dominant-negative mutant of Rab5 delayed this collapse of apoptotic thymocytes, showing a role for Rab5 in phagosome maturation. Disruption of microtubules with nocodazole inhibited Rab5 activation on the phagosome membrane without perturbing the engulfment of apoptotic cells. Furthermore, we found that Gapex-5 is the guanine nucleotide exchange factor essential for Rab5 activation during the engulfment of apoptotic cells. Gapex-5 was bound to a microtubule-tip-associating protein, EB1, whose depletion inhibited Rab5 activation during phagocytosis. We therefore propose a mechanistic model in which the recruitment of Gapex-5 to phagosomes through the microtubule network induces the transient Rab5 activation.

摘要

凋亡细胞的高效吞噬作用对于组织稳态和免疫反应至关重要。Rab5是早期内吞途径的关键调节因子,我们最近发现Rab5也参与凋亡细胞的吞噬;然而,Rab5活性的确切时空动态仍不清楚。在此,我们使用新开发的荧光共振能量转移生物传感器,描述了凋亡胸腺细胞吞噬过程中Rab5活性的变化。吞噬体膜上的Rab5活性在包裹吞噬体的肌动蛋白外壳解体时开始增加。Rab5激活持续或重复长达10分钟,但在被吞噬的凋亡细胞崩溃之前结束。Rab5显性负性突变体的表达延迟了凋亡胸腺细胞的这种崩溃,表明Rab5在吞噬体成熟中起作用。用诺考达唑破坏微管抑制了吞噬体膜上的Rab5激活,而不干扰凋亡细胞的吞噬。此外,我们发现Gapex-5是凋亡细胞吞噬过程中Rab5激活所必需的鸟嘌呤核苷酸交换因子。Gapex-5与微管末端相关蛋白EB1结合,EB1的缺失抑制吞噬过程中的Rab5激活。因此,我们提出了一个机制模型,即通过微管网络将Gapex-5募集到吞噬体上可诱导Rab5的瞬时激活。

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